2006
DOI: 10.1074/jbc.m512544200
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Fumarate Reductase and Succinate Oxidase Activity of Escherichia coli Complex II Homologs Are Perturbed Differently by Mutation of the Flavin Binding Domain

Abstract: The Escherichia coli complex II homologues succinate:ubiquinone oxidoreductase (SQR, SdhCDAB) and menaquinol:fumarate oxidoreductase (QFR, FrdABCD) have remarkable structural homology at their dicarboxylate binding sites. Although both SQR and QFR can catalyze the interconversion of fumarate and succinate, QFR is a much better fumarate reductase, and SQR is a better succinate oxidase. An exception to the conservation of amino acids near the dicarboxylate binding sites of the two enzymes is that there is a Glu … Show more

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Cited by 49 publications
(80 citation statements)
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“…CT amplitude does not change at pH 7 or 9 and does not correlate with the pK a of the reaction (36,49). This suggests that microscopic pK a values of amino acid residues involved in substrate activation are below pH 7, and the observed pK a of the reaction is influenced by other active site or proton shuttle residues.…”
Section: Discussionmentioning
confidence: 69%
See 1 more Smart Citation
“…CT amplitude does not change at pH 7 or 9 and does not correlate with the pK a of the reaction (36,49). This suggests that microscopic pK a values of amino acid residues involved in substrate activation are below pH 7, and the observed pK a of the reaction is influenced by other active site or proton shuttle residues.…”
Section: Discussionmentioning
confidence: 69%
“…Potassium ferricyanide and phenazine ethosulfate/2,6-dichlorophenol indophenol were used as electron acceptors for reactions of succinate oxidation for QFR and SQR, respectively (35). Fumarate reduction was determined with reduced methyl viologen or by menaquinol oxidation, as described previously (36). Optical spectra were recorded with an Agilent 8453 diode array spectrophotometer 1 min after the addition of ligand to an isolated enzyme in 30 mM BTP, 0.1 mM EDTA, 0.01% Anapoe C 12 E 9 .…”
Section: Methodsmentioning
confidence: 99%
“…314 The reduction potentials of the four centers were also determined using PFV ( Figure 26B) and found to match independent measurements. 36,38,66,278 The assumption that the centers are redox-independent was explicitly made and questioned, 36 but it should be recognized that the relatively low intensity of the peak currents observed for large multicenter enzymes often precludes the use of noncatalytic PFV to investigate the possible redox cooperativity between the different redox centers (section 2.1.1.2). Should redox interactions be suspected or detected 76 (as in multiheme cytochromes for example), it is important to think of the nontrivial relation that exists between the "macroscopic" reduction potentials measured in PFV (or UV-vis if the centers are indistinguishable for example) and their "microscopic" counterparts, which can sometimes be determined from titrations followed by NMR or EPR.…”
Section: Observing Reasonable Noncatalytic Signalsmentioning
confidence: 99%
“…This includes nanoparticles (graphite, 20 silica, 264,265 gold, [266][267][268] Pt,etc. )andnanotubes, 235,269 quantum dots, and mesoporous materials (electrodeposited oxides, 278,271 ITO, carbon, etc). The reader will find many examples in recent reviews.…”
mentioning
confidence: 99%
“…Previous analyses have suggested a role of the reduction potentials of the Fe-S clusters, the properties of the covalently bound FAD cofactor, and quinone substrates in catalytic proficiency (10,14,18,32). Because electrons are substrates and products, the tuning of the potentials can control substrate availability at each active site.…”
Section: Membranesmentioning
confidence: 99%